Development of a telomere vector‐based approach to overcome limitations caused by lethal phenotypes in the study of essential genes in Magnaporthe oryzae

Abstract Reverse genetic approaches are common tools in genomics for elucidating gene functions, involving techniques such as gene deletion followed by screening for aberrant phenotypes. If the generation of gene deletion mutants fails, the question arises whether the failure stems from technical issues or because the gene of interest (GOI) is essential, meaning that the deletion causes lethality. In this report, we introduce a novel method for assessing gene essentiality using the phytopathogenic ascomycete Magnaporthe oryzae. The method is based on the observation that telomere vectors are lost in transformants during cultivation without selection pressure. We tested the hypothesis that essential genes can be identified in deletion mutants co‐transformed with a telomere vector. The M. oryzae gene MoPKC, described in literature as essential, was chosen as GOI. Using CRISPR/Cas9 technology transformants with deleted GOI were generated and backed up by a telomere vector carrying a copy of the GOI and conferring fenhexamid resistance. Transformants in which the GOI deletion in the genome was not successful lost the telomere vector on media without fenhexamid. In contrast, transformants with confirmed GOI deletion retained the telomere vector even in absence of fenhexamid selection. In the latter case, the maintenance of the telomere indicates that the GOI is essential for the surveillance of the fungi, as it would have been lost otherwise. The method presented here allows to test for essentiality of genes when no mutants can be obtained from gene deletion approaches, thereby expanding the toolbox for studying gene function in ascomycetes.


| INTRODUC TI ON
Phytopathogenic fungi pose a threat to global food and raw material production, due to their potential to cause substantial economic losses.Despite progress in breeding for high-yield crop varieties and the use of fungicides, plant pathogens continue to threaten crops because they evolve resistances to certain fungicide classes (Fischer & Edmeades, 2010;McDonald & Stukenbrock, 2016;Oerke, 2006).
A silver bullet could identify essential genes in pathogens for targeted development of novel plant protection agents that would prevent the development of possible fungicide resistances (Cole, 2002).
In fungi, approximately one-fifth of the genome consists of essential genes (Decottignies et al., 2003;Winzeler et al., 1999) and their identification is described as the primary task in genome-based validation of potential drug targets (Chalker & Lunsford, 2002;Decottignies et al., 2003).Molecular genetic methods to identify and prove the essentiality of genes may involve the generation of conditional lethal mutants, for example, by point mutations (Chalker & Lunsford, 2002;Firon et al., 2002).An alternative is the activation or repression of gene expression using regulatable promoters (Cairns et al., 2016;Dichtl et al., 2012;Missall & Lodge, 2005;O'Meara et al., 2015;Roemer et al., 2003), but such promoters are potentially leaky and their applicability is restricted to certain organisms (Care et al., 1999).In Aspergillus fumigatus, insertional mutagenesis in combination with parasexual genetics has been used for the identification of essential genes (Firon et al., 2002(Firon et al., , 2003;;Ichinomiya et al., 2007).As this approach relies on a parasexual lifestyle, it is not universally applicable to other fungi.Other methods include the inhibition of protein activity, which is an elegant method but can only be applied to enzymes whose substrates are known and for which inactive analogues are available (Dang et al., 2011;Penn et al., 2015).

All of the above-mentioned methods have certain limitations
and do not provide a versatile tool for testing gene essentiality in most ascomycetes.We therefore aimed to develop a fast and efficient method using the model organism for plant-pathogenic fungi Magnaporthe oryzae.The method is based on the co-transformation of M. oryzae protoplasts using a CRISPR/Cas9-sgRNA-ribonucleoprotein (RNP)-complex together with a DNA deletion construct for targeted gene-replacement of the genomic version of the GOI and a transiently stable telomere vector containing a copy of the GOI.Telomere vectors contain telomeric sequences that prevent them from integrating into the host genome at high rates and replicate autonomously as centromere-free mini-chromosomes (Barreau et al., 1998;Javerzat et al., 1993).Previous studies have shown that plasmids containing a pair of human telomeres can be efficiently used to transform filamentous fungi and that these vectors are only stable in host cells under selection conditions (Barreau et al., 1998;Leisen et al., 2020;Perrot et al., 1987).However, the stability varies between different fungi and the use of telomere vectors prevents genomic integration, ranging from 85% in Botrytis cinerea to 100% in Podospora anserina (Barreau et al., 1998;Leisen et al., 2020).By combining the strengths of CRISPR/Cas9 technology with telomere vectors, marker-free genome editing can be achieved, as it has been reported for the fungi B. cinerea and M. oryzae (Leisen et al., 2020).While telomere vectors are lost at high percentages under nonselective growth conditions, we speculated that such a vector would be maintained if it encodes an expression cassette for an essential gene that is simultaneously deleted during the transformation process in the genome (Figure 1).To test this hypothesis, the M. oryzae gene MoPKC was chosen; this encodes a protein kinase C, an enzyme belonging to the serine/threonine kinase family, that is found in all eukaryotes (Penn et al., 2015).The MoPkc protein is involved in signalling related to growth, development and cell death and has been reported as a gene essential for the viability of M. oryzae (Penn et al., 2015).Results presented here indicate that the telomere vector carrying the MoPKC gene did not get lost, even under nonselective conditions, in mutants in which the same gene F I G U R E 1 Schematic presentation of the strategy for identification of essential genes.Protoplasts are co-transformed with a CRISPR/Cas9-sgRNA-ribonucleoprotein (RNP)-complex, a gene-deletion construct (Hyg R -RT) and the telomere vector pTEL-Fen::GOI, encoding the gene of interest (GOI) under the control of a constitutive promoter.The RNP and Hyg R -RT are used to perform targeted deletion of the GOI in the genome.A telomere vector encoding the same GOI and a fenhexamid-resistant cassette is additionally cotransformed.The telomere vector is only maintained in transformants during selection with fenhexamid and gets lost without selection pressure.However, if the GOI, provided on the telomere vector and deleted in the genome, is essential for the viability of the fungus, the telomere vector is stable in transformants even on medium without fenhexamid.Thereafter, testing of transformants for fenhexamid resistance will only be successful if the GOI is an essential gene and thus the telomere vector is maintained.
was simultaneously deleted on the chromosome.Our findings were further exemplified by using the MoALB1 gene, whose deletion results in a whitish phenotype and serves as an easily traceable marker for assessing the loss or maintenance of telomere vectors.

| RE SULTS
The approach towards establishing a novel tool for the study of essential genes in ascomycetes encompassed two consecutive steps: the first to demonstrate that telomere vectors get lost during cultivation of transformants without selection pressure over a considerable time period, and the second to show that such a vector is maintained when it encodes an essential gene that has simultaneously been deleted in the genome of the target organism.As a case study, we chose M. oryzae, a well-established model organism for plant-pathogenic fungi, and selected two functionally characterized genes.The loss of one of these genes could be easily traced back due to a colour-changed phenotype (MoALB1) and the second encodes a protein kinase C (MoPkc) known to be essential for viability of the fungus.

| Telomere vectors get lost without selection pressure
Mycelium of wild-type M. oryzae isolate Guy11 appears brownish when grown on complete medium (CM).Deletion of the gene MoALB1 (MGG_07219), which encodes a polyketide synthase that is involved in melanin biosynthesis, results in a whitish appearance of the mycelium (Foster et al., 2018) (Figure 2a).We transformed protoplasts of a whitish mutant (∆Moalb1) with the telomere vector pTEL-Fen::MoALB1, which carries the wild-type MoALB1 gene under the control of the constitutive Prbp27 promoter and a gene conferring resistance to fenhexamid (fen) (Wegner et al., 2022).After initial selection with fen, mutants were transferred to nonselective CM.The brownish colour of the mycelium of these mutants indicated the complementation of ∆Moalb1 with the wild-type gene provided on the telomere vector.After 1 week of cultivation on CM without fen, the mutant colonies had a brownish centre and whitish hyphae at the outer border, corresponding to the oldest and youngest parts of a growing colony, respectively (Figure 2b-I).We concluded that the telomere vector, with the wildtype MoALB1 gene, had got lost in the youngest parts of the colonies during cultivation for 1 week.To test this hypothesis, we transferred F I G U R E 2 Loss of pTEL-Fen::MoALB1 in the absence of selection pressure.(a) While mycelium of Magnaporthe oryzae isolate Guy11 is brownish, the deletion of MoALB1 results in a whitish phenotype.(b) Protoplasts of Moalb1 mutant were transformed with the telomere vector pTEL-Fen::MoALB1.After initial selection with fenhexamid (fen), ΔMoalb1::pTEL-Fen::MoALB1 transformants were cultivated for 2 weeks on nonselective complete medium (CM).After 1 week (colony diameter 2 cm), mycelium from the border of a colony was transferred to new CM plate.While the mycelium of the transformants appeared brown immediately after selection (I), it became white without selection pressure (II), indicating the loss of the telomere vector pTEL-Fen::MoALB1.After cultivation without selection pressure for 2 weeks, transformants were transferred to CM or CM + fen (III).Tested transformants grew with whitish mycelium on CM and no growth occurred on fenhexamid-containing medium, both confirming the loss of the telomere vector pTEL-Fen::MoALB1.(c) In four independent experiments, 16 fen R transformants were analysed with regard to fenhexamid sensitivity or resistance after cultivation on nonselective medium for 2 weeks.In each experiment, all of the 16 transformants lost fenhexamid resistance, that is, the telomere vector pTEL-Fen::MoALB1.white mycelium from the border of 16 colonies to CM without fen and cultivated it for another week.The entire mycelium of all 16 colonies had a whitish colour (Figure 2b-II), confirming that the telomere vector with the wild-type MoALB1 gene was lost.To further corroborate this conclusion, colonies from the latter plate were transferred to either CM or CM + fen and cultivated for another week (Figure 2b-III).While colonies on CM plates grew with a whitish mycelium, no growth was observed on CM + fen.This unequivocally showed that the telomere vector (pTEL-Fen::MoAlb1), which also carried the gene conferring fen resistance, had been lost during cultivation on CM without fen.We performed four independent replicates of the above-described transformation experiment and selected in each case 16 mutants with fen (Figure 2c).Cultivation of these 16 mutants on CM without fen resulted in the loss of fen resistance, at a rate of 100%.With these results the first requirement for the proposed assay, the loss of telomere vectors without selection pressure, was fulfilled.

| Co-transformation with pTEL-Fen::MoPKC enables deletion of the essential gene MoPKC
Next, we selected MoPKC, a gene reported in the literature to be essential for growth of M. oryzae (Penn et al., 2015), as candidate for the proof-of-concept experiments.In this assay, we aimed to delete the genomic copy of MoPKC and concurrently provide the sequence of the wild-type gene, in an analogous approach as described above for MoALB1, on a telomere vector (pTEL-Fen::MoPKC).The targeted deletion was achieved by inducing a DNA double-strand break (DSB) upstream of the gene MoPKC using a CRISPR/Cas9-RNP as described in Leisen et al. (2020).By targeting this region upstream of the gene, the Cas9-endonuclease was kept from cleaving the MoPKC gene copy provided on the telomere vector.For transformation of M. oryzae protoplasts, the Cas9 4×SV40 was mixed with the sgRNA and a template containing the hygromycin (hyg) resistance-encoding gene hph for replacement of the genomic version of MoPKC.
At first, we deleted MoPKC in the wild-type Guy11 isolate and added a telomere vector with a gene cassette providing fen resistance but without the MoPKC gene (pTEL-Fen).Co-selection on hyg and fen-containing medium resulted in a total of 468 mutants (Figure 3a).However, PCR analysis and sequencing of the MoPKC locus for selected mutants revealed for none of them homologous integration of the hygromycin-resistance cassette at the MoPKC wild-type locus.For improvement, we did the same transformation in the MoΔku80 genotype, a mutant known to be impaired in nonhomologous end-joining (NHEJ) (Villalba et al., 2008).In this case, no fen-resistant transformants were obtained when using the abovementioned telomere vector without the MoPKC gene (pTEL-Fen) (Figure 3a).This led us to speculate that in the case of the MoΔku80 genotype, deletion of the genomic version of the MoPKC gene has occurred, that is, homologous integration of the hygromycinresistance cassette was successful, and thus mutants died.
Because interpretations drawn from such indirect evidence are challenging to trace back, we next conducted an analogous experiment with a telomere vector carrying the MoPKC gene (pTEL-Fen::MoPKC).
Firstly, we verified that neither Guy11 nor MoΔku80 were able to grow on CM + fen, which was in accordance with Wegner et al. (2022) (Figure 3b).Next both genotypes, Guy11 and MoΔku80, were transformed with pTEL-Fen::MoPKC but in the absence of CRISPR/Cas9, meaning that the MoPKC gene will not be deleted in the genome (Figure 3b).Mutants that had taken up the telomere vector were initially selected on CM + fen, transferred to CM without fen and further cultivated for 2 weeks.Thereafter, mutants were rescreened F I G U R E 3 Co-transformation of pTEL-Fen::MoPKC enables deletion of the essential gene MoPKC in the genome.(a) Guy11 and MoΔku80 protoplasts were co-transformed with a Cas9-sgRNA-RNP targeting the native locus of MoPKC, a Hyg R -RT and the telomere vector pTEL-Fen.When using Magnaporthe oryzae Guy11, 468 transformants were generated, but for none of them deletion of MoPKC was confirmed.When using the nonhomologous end-joining-deficient mutant MoΔku80, no fenhexamid-resistant (fen R ) transformants were generated.(b) Transfer of the wild-type strain Guy11 and the mutant MoΔku80 from complete medium (CM) to CM + fen indicated that they are not resistant to this fungicide.Protoplasts of M. oryzae Guy11 and MoΔku80 were transformed with the telomere vector pTEL-Fen::MoPKC but without deletion of MoPKC on the genome.Sixteen fen R Guy11 or MoΔku80 transformants were initially transferred to CM + fen, followed by cultivation on CM without fen for 2 weeks and then transferred again to CM + fen.(c) Across four independent experiments, 14-16 fen R Guy11 transformants were tested for fen-sensitivity/resistance after cultivation on CM without fen for 2 weeks.For MoΔku80, 16-32 fen R transformants were analysed in two independent experiments.On average, 87% of the tested Guy11 transformants and 86% of the MoΔku80 transformants lost fenhexamid resistance, along with the telomere vector pTEL-Fen::MoPKC, after cultivation on CM without fen.(d) Protoplasts of M. oryzae Guy11 and MoΔku80 were co-transformed with the Cas9-sgRNA-RNP, the Hyg R -repair template and the telomere vector pTEL-Fen::MoPKC.After initial selection with fen and hygromycin (hyg), 14-16 fen R + hyg R Guy11 and MoΔku80 transformants were transferred to CM + fen, and subsequently cultivated on CM without fen for 2 weeks and then retransferred to CM + fen.All confirmed ΔMopkc transformants were able to grow on the selective medium.(e) Fifteen or 16 fen R + hyg R Guy11 transformants were tested in quadruplicate for deletion of the genomic version of the MoPKC gene and fen resistance after 2 weeks of cultivation on CM without fen.In mutants in which PCR analysis confirmed deletion of MoPKC by homologous recombination, no loss of fen resistance had occurred, meaning that the telomere vector pTEL-Fen::MoPKC was still present.In three independent experiments, 14-16 fen R + hyg R transformants of MoΔku80 were analysed for MoPKC deletion and resistance to fen.Consistent with findings for Guy11, mutants with confirmed MoPKC deletion did maintain the telomere vector pTEL-Fen::MoPKC and thus fen resistance.(f) Average deletion rates via homologous recombination in Guy11 and MoΔku80.Values are calculated as ratio of transformants with confirmed MoPKC deletion relative to all tested fen R + hyg R transformants (Figure 4e).Bars display the average and standard deviation calculated from four and three independent experiments for Guy11 and MoΔku80, respectively.The level of significance was determined using t test.
on CM + fen (Figure 3b).Almost all mutants did not survive fen selection, indicating the loss of the telomere vector during cultivation without selection pressure.This loss occurred with a frequency of 80%-94% or 84%-88% in the Guy11 and MoΔku80 genotypes, respectively (Figure 3c).For the few mutants that survived the final selection, it must be concluded that the fen-resistance cassette had integrated into the genome.Next, both M. oryzae genotypes were to 9/14.This highlighted the significantly better gene deletion rate for the M. oryzae genotype MoΔku80, with disabled NHEJ, compared to Guy11 at 73% and 24%, respectively (Figure 3f).The mutants with confirmed deletion of MoPKC in the genome were cultivated further for 2 weeks on CM without fen and thereafter rescreened on CM + fen (Figure 3d).None of these mutants lost the ability to grow on fen-containing medium (Figure 3e), indicating the maintenance of the telomere vector even in absence of selection pressure.In other words, these results demonstrate that in mutants where the MoPKC gene has successfully been deleted in the genome, an otherwise instable telomere vector is maintained when it carries an expression cassette for the same gene.

| DISCUSS ION
Telomere vectors in combination with the CRISPR/Cas9 technology have already been reported as powerful tools to achieve marker-free genome editing in M. oryzae (Leisen et al., 2020).Building on these results, a pTEL-Fen and CRISPR/Cas9-mediated strategy for verification of essential genes in ascomycetes was established in this study.
The basis for this strategy is the observation that telomere vectors conferring fen resistance get lost after transformation under nonselective growth conditions, as shown for M. oryzae ∆Moalb1 (Figure 2).This mutant was particularly useful because it has a whitish mycelium that could be complemented with a telomere vector containing the wild-type MoALB1 gene and thus mycelium colour changed to the wild-type (brown) phenotype.The loss of the telomere vector was easily visible by monitoring the occurrence of colonies with whitish mycelium in the absence of fen selection.To demonstrate that such a vector becomes stable when it contains a functional copy of an essential gene, we performed a co-transformation assay in which the deletion of GOI (MoPKC) on the chromosome and the substitution with a GOI copy on a telomere vector was achieved simultaneously.
The respective telomere vector (pTEL-Fen::MoPKC) was lost in at least 86% of the selected transformants after 2 weeks of cultivation on nonselective medium when the gene was not simultaneously deleted in the genome (Figure 3).This underpins that fungal genes on telomere vectors do not integrate into the genome, or at least are prevented from doing so at high percentages, thus supporting similar findings reported by Perrot et al. (1987), Barreau et al. (1998) and Leisen et al. (2020).Co-transformation of the M. oryzae isolate Guy11 and the Mo∆ku80 mutant with pTEL-Fen::MoPKC, the in vitro assembled CRISPR/Cas9-sgRNA complex and the MoPKC-deletion construct resulted in a high rate of transformants similar to that described in Leisen et al. (2020).PCR analysis of selected transformants revealed significantly higher rates of homologous integration, resulting in deletion of MoPKC on the chromosome, in the NHEJ-deficient mutant Mo∆ku80 (Figure 3a).These high editing rates were achieved with microflanks for homologous recombination, as described by Foster et al. (2018), which reconfirmed the improvement by avoiding cloning of 1000 bp long homologous flanks.Transformants with a deletion of MoPKC in the genome maintained the telomere vector pTEL-Fen::MoPKC, even if F I G U R E 4 PCR-based approach to confirm MoPKC gene deletion.Schematic setup of MoPKC-gene-deletion by using CRISPR/Cas9mediated genome editing and homologous recombination (HR) to replace MoPKC by the resistance marker gene hph.Because MoPKC deletion is lethal, MoPKC must be simultaneously provided on a telomere vector (not shown) to generate Magnaporthe oryzae transformants.A double-strand break (DSB) was induced upstream of the MoPKC gene by the Cas9-sgRNA-ribonucleoprotein (RNP).By targeting the sequence upstream of MoPKC, the Cas9-endonuclease is prevented from cutting the copy of MoPKC provided on the telomere vector.The DSB caused by the Cas9-endonuclease facilitates the integration of the Hyg R -repair template (RT) into the genome through HR, resulting in the deletion of MoPKC.A nucleotide sequence of 94 bp at the 3′-end of the gene will be maintained.In order to verify HR between MoPKC and Hyg R -RT, primer combinations MoPKC_cleavage-for/rev, MoPKC_cleavage-for/HG-rev, HY-for/MoPKC_FL-rev and MoPKC_KO1-for/rev were used for PCR analysis.Only if all four PCR products were amplified with calculated product sizes was the respective mutant considered as a successful gene deletion mutant.cultivated on nonselective medium (CM without fen) for several weeks (Figure 3e).Conversely, when co-transforming M. oryzae protoplasts with pTEL-Fen::MoPKC but without MoPKC-deletion construct, the telomere vector was not maintained but rather got lost after a few weeks (Figure 3b,c).However, due to the low rate of genome integration observed with telomere vectors, the approach should always include a concurrent PCR analysis to confirm the fate of the telomere vector.In accordance with the study of Penn et al. (2015), these results emphasize the essential role of MoPKC for the viability of M. oryzae.Furthermore, our strategy of using a pTEL-Fen and CRISPR/Cas9-mediated genome editing to verify essential genes in ascomycetes has thus been successfully established.It should be noted that the use of the constitutive promoter Prbp27 might cause problems if the native gene expression pattern significantly differs from that of the constitutive promoter.In this case, the use of the native promoter sequence of the respective gene should be considered.Consequently, it would be necessary to target a sequence the Cas-9-RNP in the sequence upstream of the promoter or downstream of the terminator region.However, when dealing with gene dosage effects, it should also be carefully considered that the copy number of the telomere vector was determined to be lower than the chromosomal copy number, at least in B. cinerea (Leisen et al., 2020), which could also have an impact on the gene dosage effect.Apart from M. oryzae, the telomeric nucleotide sequence (T 2 AG 2 ) n is conserved in many other filamentous fungi such as Fusarium oxysporum, Podospora anserina, Cladosporium fulvum, Aspergillus nidulans and Neurospora crassa (Bhattacharyya, 1997;Coleman et al., 1993;Farman & Leong, 1995;Javerzat et al., 1993;Powell & Kistler, 1990;Schechtman, 1990).In addition, high transformation frequencies and autonomous replication of linear DNA molecules with telomeric ends have already been achieved in F. oxysporum, Histoplasma capsulatum, Nectria haematococca, Cryprococcus neoformans, P. anserina and B. cinerea (Kistler & Benny, 1992;Powell & Kistler, 1990;Woods & Goldman, 1992).Based on these findings, the combination of efficient CRISPR/Cas9-technology with non-integrative vectors containing human telomeres (telomere vectors) represents a promising approach for verification of essential genes, not only in M. oryzae, but also in perspective, in filamentous fungi in general.This provides a strategy to determine whether the absence of mutants in a gene deletion approach is due to the essential role of the target gene or to a failure of gene replacement.

| Fungal isolates of M. oryzae
M. oryzae Guy11 and the MoΔku80 mutant were provided by D.
Tharreau from CIRAD (Montpellier, France) and were cultivated on complete medium (CM), supplemented with agar, at a temperature of 23°C in absence of light (Talbot et al., 1993).

| Vector construction
The vector pTEL-Fen-MCS (File S1), which was used as starting vector in this study, was obtained by cloning the expression cassette of pTK144-MCS (Prbp27-MCS-Stop-mRFP-TtubB) (pTK144 provided by Thomas Kroj, INRA, UMR BGPI, Montpellier, France) into the telomere vector pTEL-Fen (provided by Matthias Hahn, TU, Kaiserslautern, Germany) using Gibson assembly (Gibson Assembly Master Mix; New England BioLabs).Therefore, we amplified the DNA sequence of the expression cassette from the plasmid pTK144-MCS by PCR, using Phusion Hot Start High Fidelity DNA polymerase (Thermo Fisher Scientific) and the primer pair pTK144-OE_for/ rev (Table S1).Next, the PCR product of the overexpression construct was purified using the NucleoSpin gel and PCR clean-up kit (Macherey-Nagel).The vector was restricted with BamHI/KpnI (fast digest enzymes, Thermo Fisher Scientific) and then the overexpression cassette was inserted using Gibson assembly.Afterwards, the ligated plasmid (pTEL-Fen-MCS) was used for transformation of Escherichia coli DH5α (Thermo Fisher Scientific).The vector was purified from E. coli using the NucleoSpin Plasmid Kit (Macherey-Nagel) and verified by sequencing (Microsynth SeqLab, Göttingen, Germany).
To generate the vectors pTEL-Fen::MoALB1 and pTEL-Fen::MoPKC (File S1), the previously generated telomere vector pTEL-Fen-MCS was digested with BcuI and KpnI.The coding sequences of MoPKC (MGG_08689) and MoALB1 (MGG_07219) were amplified by PCR from genomic DNA of M. oryzae wild-type isolate Guy11 using Phusion Hot Start High Fidelity DNA polymerase and the primer pairs PKC_MCS-for/rev and ALB_MCS-for/rev, respectively.
Primers were designed with respective overlapping sequence to pTEL-Fen-MCS (Table S1).The PCR products were purified using the NucleoSpin Gel and PCR clean-up kits and cloned into the BcuI/ KpnI-restricted telomere vector pTEL-Fen-MCS by Gibson assembly.Through this step, the genes were set under the control of the constitutive expression promoter Prbp27.The ligated vector was transformed into E. coli.Vectors were purified from E. coli using the NucleoSpin plasmid kit and successful insertion of the targeted genes into pTEL-Fen was confirmed by sequencing.
Oligonucleotides used for synthesis of sgRNA (gRNA_MoALB1/ gRNA_konst.) are listed in Table S1.The ΔMoalb1 mutant was generated by mixing 120 μL of the protoplast suspension of M. oryzae isolate Guy11 with 6 μg Cas9-RNP targeting MoALB1 and 6 μg repair template (RT) suspended in a total volume of 60 μL Tris-CaCl 2 buffer.
co-transformed with pTEL-Fen::MoPKC, the Cas9-sgRNA-RNP and a gene deletion construct for the genomic version of MoPKC.Again, an initial selection of transformants was done on fen-containing medium and selected mutants were tested by sequencing of respective PCR products for deletion of MoPKC in the genome (Figure3d).In four independent biological replicates for Guy11, the gene deletion rate varied from 2/16 to 5/15 and for the MoΔku80 genotype from 13/16